Enhancing biosynthesis of 2'-Fucosyllactose in Escherichia coli through engineering lactose operon for lactose transport and alpha-1,2-Fucosyltransferase for solubility

被引:23
|
作者
Park, Bum Seok [1 ,2 ]
Choi, Yun Hee [2 ,3 ]
Kim, Min Woo [2 ,3 ]
Park, Beom Gi [1 ,2 ]
Kim, Eun-Jung [4 ]
Kim, Jin Young [2 ,3 ]
Kim, Jung Hwa [1 ,3 ]
Kim, Byung-Gee [1 ,2 ,3 ,4 ,5 ]
机构
[1] Seoul Natl Univ, Sch Chem & Biol Engn, Seoul 08826, South Korea
[2] Seoul Natl Univ, Inst Mol Biol & Genet, Seoul, South Korea
[3] Seoul Natl Univ, Interdisciplinary Program Biochem Engn & Biotech, Seoul, South Korea
[4] Seoul Natl Univ, Bio MAX N Bio Inst, Seoul, South Korea
[5] Seoul Natl Univ, Inst Sustainable Dev ISD, Seoul, South Korea
基金
新加坡国家研究基金会;
关键词
Escherichia coli; Fucosyllactose; Fucosyltransferase; metabolic engineering; protein engineering; HUMAN-MILK OLIGOSACCHARIDE; 2'-FUCOSYLLACTOSE; 3-FUCOSYLLACTOSE; PATHWAY;
D O I
10.1002/bit.28048
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
2'-Fucosyllactose (2'-FL) is the most abundant oligosaccharide in human milk and one of the most actively studied human milk oligosaccharides (HMOs). When 2'-FL is produced through biological production using a microorganism, like Escherichia coli, d-lactose is often externally fed as an acceptor substrate for fucosyltransferase (FT). When d-glucose is used as a carbon source for the cell growth and d-lactose is transported by lactose permease (LacY) in lac operon, d-lactose transport is under the control of catabolite repression (CR), limiting the supply of d-lactose for FT reaction in the cell, hence decreasing the production of 2'-FL. In this study, a remarkable increase of 2'-FL production was achieved by relieving the CR from the lac operon of the host E. coli BL21 and introducing adequate site-specific mutations into alpha-1,2-FT (FutC) for enhancement of catalytic activity and solubility. For the host engineering, the native lac promoter (P-lac) was substituted for tac promoter (P-tac), so that the lac operon could be turned on, but not subjected to CR by high d-glucose concentration. Next, for protein engineering of FutC, family multiple sequence analysis for conserved amino acid sequences and protein-ligand substrate docking analysis led us to find several mutation sites, which could increase the solubility of FutC and its activity. As a result, a combination of four mutation sites (F40S/Q150H/C151R/Q239S) was identified as the best candidate, and the quadruple mutant of FutC enhanced 2'-FL titer by 2.4-fold. When the above-mentioned E. coli mutant host transformed with the quadruple mutant of futC was subjected to fed-batch culture, 40 g l(-1) of 2'-FL titer was achieved with the productivity of 0.55 g l(-1) h(-1) and the specific 2'-FL yield of 1.0 g g(-1) dry cell weight.
引用
收藏
页码:1264 / 1277
页数:14
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